Effects of mannan oligosaccharide supplementation on growth, some immune responses and gut lactic acid bacteria of common carp (Cyprinus Carpio) fingerlings.

This study was conducted to determine the effects of mannan oligosaccharide (MOS) on growth, some immune responses and gut lactic acid bacteria of common carp. Four experimental diets containing 0%, 0.05%, 0.10% and 0.20% MOS were prepared. Each diet was randomly allocated to triplicate groups of fish with initial average weight of approximately 14 g. After eight weeks, survival rate was high in all treatments with no significant difference (p > 0.05). Growth performance including final weight, weight gain (WG) and specific growth rate (SGR) did not differ among the treatments. Feed conversion ratio (FCR) was better when the fish were fed 0.05 to 0.20% MOS diets. The alternative complement activity, lysozyme activity and serum total Ig were found to be significantly (p < 0.05) greater in fish fed 0.20% MOS diets. Although the total intestinal bacterial counts were not affected by dietary treatment (p > 0.05), the lactic acid bacteria levels were significantly elevated in fish fed MOS diets (p < 0.05). These results indicated that oral administration of MOS at 0.20% elevated the immune response, improved FCR and modulated intestinal microbiota of common carp.


Introduction
Antibiotics, for the past decades, have been included at the sub-therapeutic concentrations in the aqua-feeds due to their potential effects on survival, feed utilization and weight gain. 1 However, with the recent ban on the use of antibiotic growth promoters as additives in fish feed, alternative immunonutriens to enhance production and health status is a research topic of increasing interest. Prebiotics which are defined as non-digestible food ingredients beneficially affect the host by stimulating growth and/or activity of a limited number of beneficial bacteria in the gastrointestinal tract and have proved to be effective at enhancing health and growth performance of terrestrial and aquatic animals. 2 Among the most common prebiotics, mannan oligosaccharide (MOS) has been recently receiving heightening application in aquaculture. 1 The MOS are complex carbohydrates derived from yeast cell walls. These compounds contain mannose as the primary carbohydrate element. 3 This prebiotic has been demonstrated to have a variety of beneficial effects on livestock ranging from growth enhancing to immunostimulation in many species. 4 The growth promotion [5][6][7] and immunostimulatory benefits 8,9 of dietary MOS have also been studied in fish but often with contrasting findings.
The culture of warm-water species is an important aquaculture industry in Iran. Warm-water fish farming in Iran is based on Chinese carps including common carp (Cyprinus carpio). Annual production of farmed carps in Iran was 100,430 tons in 2009. 10 The present study was carried out to investigate the effects of dietary MOS supplementation on the growth performance and immunological parameters of common carp.

Materials and Methods
Fish and experimental conditions. Three hundred common carp fingerlings were obtained from a commercial carp farm in Shoushtar, Iran. The fish were transported to the laboratory, acclimated to laboratory conditions and fed the basal experimental diet without dietary MOS for one week. At the end of the acclimation period, fish with an average weight of approximately 14 g were randomly selected and stocked in twelve 300-L tanks (triplicate groups per dietary treatment) at a density of 20 fish per tank. The mean water quality parameters were recorded as follows: temperature 27 °C , dissolved oxygen 8.2 mg L -1 and pH 7.9.
Feed and feeding. Basal diet formulation and proximate composition analysis are shown in Table 1. The experimental diet was formulated to have 0% (basal), 0.05%, 0.10% and 0.20% of mannan oligosaccaride (MOS; Alltech Inc., Nicholasville, USA). Dietary ingredients were thoroughly mixed in a mixer, made into pellets and air-dried at room temperature. The pellets were broken into small pieces, packed and stored in a freezer until used.
Fish were fed by hand to apparent satiation two times per day with one of the four experimental diets over eight weeks.
Growth measurements. All fish in the different experimental groups were weighed at the end of 8-week feeding trial for estimation of growth. Based on recording the weight of each fish, specific growth rate (SGR), percentage of body weight gain (WG) and feed conversion ratio (FCR) were calculated for each group as follows: In addition, survival rate was calculated at the end of the experiment as: where, N0 is the initial number of fish and Nf is the final number of fish.  Immunological assays. After eight weeks of feeding, blood samples for serum biochemical analysis were collected from the caudal vein of nine fish per each dietary treatment into Eppendorf tubes (Eppendorf, Hamburg, Germany) without anticoagulant. Blood samples in Eppendorf tubes were allowed to clot for 30 min at room temperature. The tubes were then centrifuged at 3500 g for 5 min and the supernatant serum was collected. The serum was kept frozen at -20 ˚C until analysis of selected biochemical parameters.
Alternative complement activity (ACH50). The 50% hemolysis was determined using the method of Sunyer and Tort 11 with the following modifications as described by Yeh et al. 12 The volume of serum complement producing ACH50 was determined, and the number of ACH50 unit mL -1 was calculated for the sample.
Lysozyme activity. Lysozyme activity in serum was determined according to the method of Demers and Bayne 13 based on the lysis of the lysozyme sensitive Gram positive bacterium, Micrococcus lysodeikticus (Sigma Chemical Co., St Louis, MO, USA). The dilutions of hen egg white lysozyme (Sigma Chemical Co.) ranging from 0 to 20 µL mL -1 in 0.1 M phosphate citrate buffer (Merck, Darmstadt, Germany), pH 5.8, were taken as the standard. This along with the undiluted serum sample (25 µL) was placed into wells of a 96-well plate in triplicate. A volume of 175 µL of M. lysodeikticus suspension (75 mg mL -1 ) prepared in the same buffer was then added to each well. After rapid mixing, the change in turbidity was measured every 30 sec for 5 min at 450 nm at approximately 20 °C using a microplate reader (Model Stat Fax-2100; Awareness Technology, Palm City, USA).
Total immunoglobulin content. Plasma total immunoglobulin (Ig) level was determined according to the method described by Puangkaew et al. 14 The assay was based on the measurement of total protein content in plasma prior to and after precipitating the Ig molecules employing a 12.0% solution of polyethylene glycol (Sigma Chemical Co.). The difference in protein content represents the Ig content.
Intestinal lactic acid bacteria analysis. The analysis of intestinal microbiota was performed at the end of the feeding trial as described by Hoseinifar et al. 15 with some modifications. Four fish per tank were randomly sampled from each treatment for microbiological sampling. The fish were killed by physical destruction of the brain, and the skin was then washed in a solution of 0.10% benzalkonium chloride before opening the ventral surface with sterile scissors. Intestinal tract samples of fish were removed, weighed, and suspended in sterile 0.85% NaCl solution (Merck, Darmstadt, Germany) and homogenized. The suspension, serially diluted to 10 -6 and 20 µL of the solution was spread in triplicate on to nutrient agar (NA; Acumedia Neogen Co., Lansing, USA). Man Rogosa and Sharpe media (MRS; Quelab, Montreal, Canada) was also used to detect lactic acid bacteria (LAB). All of the plates were incubated at 36 ˚C for three days and colony forming units (CFU) per g were calculated.
Statistical analysis. The data (Mean ± standard error) were analyzed by one way analysis of variance (ANOVA) followed by Tukey's test to compare the means between individual treatments with SPSS (Version 16; SPSS Inc., Chicago, USA) at p < 0.05 level.

Results
Survival and growth measurements. At the end of trial, survival rate was high in all treatments with no significant difference (p > 0.05). The growth performance of common carp fingerlings fed diets supplemented with different levels of dietary MOS is presented in Table 2. After eight weeks of feeding, growth performance including final weight, WG and SGR did not differ among the dietary treatments, however, FCR was better when the fish were fed 0.05 to 0.20% MOS supplemented diets.
Immunological assays. The effects of the MOS on the humoral innate immune responses of common carp are shown in Figs. 1, 2, and 3. All immune parameters measured (lysozyme activity, Ig and alternative pathway of complement activity) were significantly higher (p < 0.05) in 0.2% MOS fed fish compared to the control group. Fish fed 0.20% MOS showed significantly elevated lysozyme activity compared to the control, but the activity was not significantly higher than the 0.05% and 0.10% MOS groups, as was also the case for plasma Ig and ACH50 levels.
Intestinal microbiota. Intestinal microbiota data are shown in Fig. 4. At the end of feeding trial, total bacterial levels were not affected by MOS (p > 0.05). Levels of LAB were significantly elevated in MOS fed fish compared to the control group (p < 0.05).

Discussion
This study was conducted in order to investigate the effects of MOS on growth, survival and immune responses of common carp. From previous studies it appears that the effects of MOS on growth performance of aquatic species are contradictory. The results of the current study indicate In commercial aquaculture, the farmed species are vulnerable to ubiquitous opportunistic bacterial pathogens and stimulation of the innate immune system through dietary supplements is of great interest. The alternative pathway of complement activity acts as a powerful nonspecific defense mechanism, protecting fish from a wide range of potentially invasive organisms, such as bacteria, fungi, viruses, and parasites. 21 Lysozyme, being an enzyme with antimicrobial activity, can split peptidoglycan in Control 0.05 0.1 0.2 bacterial cell walls especially of the Gram positive species and can cause lysis of the cells. 22 As presented in Figs. 1 and 3, fish fed 0.20% MOS for eight weeks showed increased lysozyme activity and ACH50. Additionally, increased level of serum total Ig as the major components of the humoral immune system was detected in the serum of fish fed 0.20% MOS (Fig. 2). The results are consistent with findings of previous studies on shellfish 1,23 and fish species. Staykov et al. reported higher levels of bactericidal activity, lysozyme, antibody levels and alternative complement activity in rainbow trout fed MOS. 19 In addition, similar results have also been demonstrated in European sea bass fed 0.40% MOS supplemented diets. 20 Similarly, other prebiotics such as inulin and fructo-oligosaccharide (FOS) have been demonstrated to improve the innate immune response in other fish species. 15,24,25 The positive effects of prebiotics on humoral immune responses may be attributable to improved growth of health-promoting bacteria such as Lactobacillus and Bifidobacter spp. that consequently limit potentially pathogenic bacteria. 2 Our results based on analysis of intestinal microbiota revealed that LAB levels were significantly elevated in fish fed dietary MOS (p < 0.05). Prebiotics including MOS have been reported to enhance the growth of beneficial bacteria such as LAB. 2 Regarding the improvement of innate immune parameters measured in our study, it can be concluded that modulation of the intestinal microbiota towards a potentially more beneficial microbial community (i.e. elevated LAB levels) can be achieved through administration of dietary MOS.
In conclusion, the results of this study show that oral administration of MOS at 0.05-0.20% improves FCR, modulates intestinal microbiota and at 0.20% elevates the humoral immune response of common carp by increasing the alternative complement activity, lysozyme activity and serum total immunoglobin.